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秘鲁首次报道寄生拟茎点霉引起葡萄皮氏病

First Report of Phaeoacremonium parasiticum Causing Petri Disease of Grapevine in Peru.

作者信息

Romero-Rivas L C, Álvarez L A, Gramaje D, Armengol J, Cadenas-Giraldo C

机构信息

Universidad Nacional Daniel Alcides Carrión, Oxapampa, Pasco, Peru.

Instituto Agroforestal Mediterráneo, Universidad Politécnica de Valencia, Camino de Vera s/n, 46022 Valencia, Spain.

出版信息

Plant Dis. 2009 Feb;93(2):200. doi: 10.1094/PDIS-93-2-0200B.

Abstract

Since 2005, symptoms of grapevine decline have been observed on 4- to 8-month-old grapevines (cvs. Red globe and Crimson) grafted onto 1103 P rootstock in Ica and Pisco valleys in southern Peru. Affected plants exhibited weak growth, interveinal chlorosis, necrosis and wilting of leaves, and death. Dark brown-to-black streaking of the xylem was seen when transverse or longitudinal cuts were made in the trunk and shoots. Symptomatic plants were collected and sections (5 cm long) were cut from the zone between the rootstock and the scion, surface sterilized for 1 min in a 1.5% sodium hypochlorite solution, and washed twice with sterile distilled water. The sections were split longitudinally, and small pieces of discolored tissues were placed onto potato dextrose agar (PDA) supplemented with oxytetracycline (500 mg liter). Plates were incubated at 25°C in the dark for 15 days. A Phaeoacremonium sp. was consistently isolated from necrotic tissues. Single conidial isolates were obtained and grown on PDA and malt extract agar (MEA) in the dark at 25°C for 3 weeks until colonies produced spores (3). Colonies were brown on PDA and olive brown on MEA. Conidiophores were branched, 27.5 to 67.5 (42.5) μm long, and often consisting of a single phialide. Conidia were hyaline, oblong ellipsoidal, 2.5 to 4.5 (3.6) μm long, and 1.2 to 1.9 (1.6) μm wide. On the basis of these characteristics, the isolates were identified as Phaeoacremonium parasiticum (Ajello, Georg & C.J.K Wang) W. Gams, Crous & M.J. Wingf. (teleomorph Togninia parasitica L. Mostert, W. Gams & Crous) (2,3). Identity of isolate Ppa-1 was confirmed by PCR-restriction fragment length polymorphism of the internal transcribed spacer region (Phaeoacremonium-specific primers Pm1-Pm2) with the restriction enzymes BssKI, EcoO109I, and HhaI (1). Additionally, the beta-tubulin gene fragment (primers T1 and Bt2b) of this isolate was sequenced (GenBank Accession No. FJ151015). The sequence was identical to the sequence of P. parasiticum (GenBank Accession No. AY328379). Pathogenicity tests were conducted using the isolate Ppa-1. Approximately 20 μl of a suspension containing 10 conidia ml was injected into the pith of four nodes on each of 10 dormant, unrooted, 15 cm long cuttings of cv. Red Globe. Four nodes on each of 10 cuttings were used as controls and injected with an equal volume of sterile distilled water. Inoculation points were covered with Parafilm. The cuttings were planted in plastic pots and maintained at 24 ± 3°C in diffuse light, watering as needed. Within 2 months of inoculation, all P. parasicitum-inoculated cuttings exhibited shoots with very poor growth with small leaves and short internodes. In the xylem vessels, black streaks identical to symptoms observed in declining vines in the vineyard were observed. Control plants did not show any of these symptoms. The fungus was reisolated from internal tissues of symptomatic shoots of all inoculated cuttings but not from the control shoots. To our knowledge, this is the first report of P. parasiticum causing young grapevine decline in Peru. References: (1) A. Aroca and R. Raposo. Appl. Environ. Microbiol. 73:2911, 2007. (2) P. W. Crous et al. Mycology 88:786, 2006. (3) L. Mostert et al. Stud. Mycol. 54:1, 2006.

摘要

自2005年以来,在秘鲁南部伊卡和皮斯科山谷中,嫁接到1103P砧木上的4至8个月大的葡萄树(品种为红地球和绯红无核)出现了葡萄树衰退症状。受影响的植株生长衰弱,叶脉间黄化,叶片坏死、萎蔫,最终死亡。对树干和新梢进行横向或纵向切割时,可见木质部有深褐色至黑色的条纹。采集有症状的植株,从砧木和接穗之间的区域切取5厘米长的切段,在1.5%次氯酸钠溶液中表面消毒1分钟,然后用无菌蒸馏水冲洗两次。将切段纵向劈开,把变色组织的小块接种到添加了土霉素(500毫克/升)的马铃薯葡萄糖琼脂(PDA)平板上。平板在25℃黑暗条件下培养15天。从坏死组织中一直分离得到一种拟顶孢霉属真菌。获得单孢分离物,在25℃黑暗条件下于PDA和麦芽提取物琼脂(MEA)上培养3周,直至菌落产生孢子(3)。菌落在PDA上为褐色,在MEA上为橄榄褐色。分生孢子梗有分支,长27.5至67.5(42.5)微米,通常由单个瓶梗组成。分生孢子透明,长椭圆形,长2.5至4.5(3.6)微米,宽1.2至1.9(1.6)微米。根据这些特征,分离物被鉴定为寄生拟顶孢霉(Ajello, Georg & C.J.K Wang)W. Gams, Crous & M.J. Wingf.(有性型为寄生托尼亚菌L. Mostert, W. Gams & Crous)(2,3)。通过使用限制性内切酶BssKI、EcoO109I和HhaI对内部转录间隔区(拟顶孢霉属特异性引物Pm1 - Pm2)进行PCR - 限制性片段长度多态性分析,证实了分离物Ppa - 1的身份(1)。此外,对该分离物的β - 微管蛋白基因片段(引物T1和Bt2b)进行了测序(GenBank登录号FJ151015)。该序列与寄生拟顶孢霉的序列(GenBank登录号AY328379)相同。使用分离物Ppa - 1进行致病性测试。将约20微升含有10个分生孢子/毫升的悬浮液注射到10株休眠、无根、15厘米长的红地球葡萄品种插条的每个插条上的四个节间的髓部。10个插条上的另外四个节间用作对照,注射等量的无菌蒸馏水。接种点用 parafilm覆盖。将插条种植在塑料盆中,保持在24±3℃的散射光下,根据需要浇水。接种后2个月内,所有接种寄生拟顶孢霉的插条的新梢生长非常差,叶片小,节间短。在木质部导管中,观察到与葡萄园衰退葡萄树中观察到的症状相同的黑色条纹。对照植株未表现出任何这些症状。从所有接种插条的有症状新梢的内部组织中重新分离出了该真菌,但对照新梢中未分离到。据我们所知,这是寄生拟顶孢霉引起秘鲁幼龄葡萄树衰退的首次报道。参考文献:(1)A. Aroca和R. Raposo。应用与环境微生物学73:2911,2007。(2)P. W. Crous等人。真菌学88:786,2006。(3)L. Mostert等人。真菌研究54:1,2006。

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